Team:BYU Provo/Notebook/SmallPhage/Summer/Period1/Exp/7.13 Phage Propagation

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'''IV) Actual Procedure/Observations'''
'''IV) Actual Procedure/Observations'''
-
: 1. Set up phage liquid culture (7.13)
+
: 1. Set up phage liquid culture - first round of propagation(7.13)
:: - phage: 4mL LB + 1mL E coli
:: - phage: 4mL LB + 1mL E coli
:: 10uL phage: 4mL LB + 1mL E coli + 10μL 5.3 phage stock
:: 10uL phage: 4mL LB + 1mL E coli + 10μL 5.3 phage stock
Line 57: Line 57:
:: :1mL phage: 4mL LB + 1mL E coli + 1mL 5.3 phage stock
:: :1mL phage: 4mL LB + 1mL E coli + 1mL 5.3 phage stock
-
: 2. Liquid culture purification (7.15)
+
: 2. Liquid culture purification - 1(7.15)
:: 1) For each infected test tubes (10uL, 100uL, 1mL), put 1mL of liquid culture into 5 eppendorf tubes.
:: 1) For each infected test tubes (10uL, 100uL, 1mL), put 1mL of liquid culture into 5 eppendorf tubes.
:: 2) Centrifuge at 3000 rpm for 5 minutes
:: 2) Centrifuge at 3000 rpm for 5 minutes
-
:: 3) Transfer supernatant into new eppendorf tubes. 5 eppendorf tubes for each phage concentration
+
:: 3) Transfer supernatant into new eppendorf tubes. 5 eppendorf tubes for each phage concentration.
:: 4) Add 100 uL of chloroform to each of the new tubes and gently shake
:: 4) Add 100 uL of chloroform to each of the new tubes and gently shake
:: 5) We labeled the purified stock as 7.15
:: 5) We labeled the purified stock as 7.15
-
: 3. Titer to determine phage concentration (7.15)
+
: 3. Titer to determine phage concentration - 1(7.15)
:: 1) For each concentration of phage, specifically 10uL, 100uL, and 1mL, 1:100 dilution series were performed to generate 0, -2, -4, -6. 1:10 dilution series were then performed to generate -7, -8, and -9.
:: 1) For each concentration of phage, specifically 10uL, 100uL, and 1mL, 1:100 dilution series were performed to generate 0, -2, -4, -6. 1:10 dilution series were then performed to generate -7, -8, and -9.
:: 2) For each dilution, a test tube was assigned to it. To each test tube, 0.75mL of BL21 liquid culture overnight was added and then transfected with 30uL of phage dilution. After 20 minutes of incubation, 7mL of x8 agar was added to each test tube and the content was then plated.
:: 2) For each dilution, a test tube was assigned to it. To each test tube, 0.75mL of BL21 liquid culture overnight was added and then transfected with 30uL of phage dilution. After 20 minutes of incubation, 7mL of x8 agar was added to each test tube and the content was then plated.
:: 3) Plates were incubated upside down for 24 hours.
:: 3) Plates were incubated upside down for 24 hours.
-
'''V) Results'''
+
: 4. Set up phage liquid culture - second round of propagation (7.17)
-
: 1. Set up phage liquid culture
+
:: - phage: 4mL LB + 1mL E coli
 +
:: 5uL phage: 4mL LB + 1mL E coli + 5μL 5.3 phage stock
 +
:: 10uL phage: 4mL LB + 1mL E coli + 10μL 5.3 phage stock
-
: 2. Liquid culture purification
+
: 5. Liquid culture purification (7.19)
-
:: 1) For each infected test tubes (10uL, 100uL, 1mL), put 1mL of liquid culture into 5 eppendorf tubes.
+
:: 1) For each infected test tubes (5uL, 10uL, 1mL), put 1mL of liquid culture into 5 eppendorf tubes.
:: 2) Centrifuge at 3000 rpm for 5 minutes
:: 2) Centrifuge at 3000 rpm for 5 minutes
-
:: 3) Transfer supernatant into new eppendorf tubes. 5 eppendorf tubes for each phage concentration
+
:: 3) Transfer supernatant into new eppendorf tubes. 5 eppendorf tubes for each phage concentration.
:: 4) Add 100 uL of chloroform to each of the new tubes and gently shake
:: 4) Add 100 uL of chloroform to each of the new tubes and gently shake
-
:: 5) We labeled the purified stock as 7.15
+
:: 5) We labeled the purified stock as 7.19
-
: 3. Titer to determine phage concentration
+
: 6. Titer to determine phage concentration (7.19)
-
:: 1) For each concentration of phage, specifically 10uL, 100uL, and 1mL, 1:100 dilution series were performed to generate 0, -2, -4, -6. 1:10 dilution series were then performed to generate -7, -8, and -9.
+
:: 1) For each concentration of phage, specifically 5uL and 10uL, 1:100 dilution series were performed to generate 0, -2, -4, -6. 1:10 dilution series were then performed to generate -7, -8, and -9.
:: 2) For each dilution, a test tube was assigned to it. To each test tube, 0.75mL of BL21 liquid culture overnight was added and then transfected with 30uL of phage dilution. After 20 minutes of incubation, 7mL of x8 agar was added to each test tube and the content was then plated.
:: 2) For each dilution, a test tube was assigned to it. To each test tube, 0.75mL of BL21 liquid culture overnight was added and then transfected with 30uL of phage dilution. After 20 minutes of incubation, 7mL of x8 agar was added to each test tube and the content was then plated.
:: 3) Plates were incubated upside down for 24 hours.
:: 3) Plates were incubated upside down for 24 hours.
 +
'''V) Results'''
 +
: 1. Set up phage liquid culture - first round of propagation
 +
 +
: 2. Titer to determine phage concentration - 1
 +
 +
: 3. Set up phage liquid culture - first round of propagation
 +
 +
: 4. Titer to determine phage concentration - 1
-
'''VI) Proposed next step'''
+
'''VI) Conclusion/Next Step
-
: We’ll use this stock to further concentrate phage. Testing whether the amount of phage added to liquid culture will affect phage titering result will be helpful.
+

Revision as of 22:15, 17 July 2013


Small Phage May - June Notebook: Experiments



Overview
March-April
May-June
July-August
September-October

7.13 Phage Propagation Experiment


I) Purpose

To amplify the 5.3 phage stock solution we have been using for mutagenesis and determine an accurate titer for future mutagenesis.


II) Expected Outcome

A purified high titer of phage. The new stock should have a higher titer than the 5.3 phage stock, which decreased in phage viability due to sitting in the fridge for 2 month.


III) Reagent Record

Chloroform from Dr. Grose’s lab; LB; E coli BL21 liquid culture overnight; x8 top agar; 5.3 phage stock


IV) Actual Procedure/Observations

1. Set up phage liquid culture - first round of propagation(7.13)
- phage: 4mL LB + 1mL E coli
10uL phage: 4mL LB + 1mL E coli + 10μL 5.3 phage stock
100uL phage: 4mL LB + 1mL E coli + 100μL 5.3 phage stock
 :1mL phage: 4mL LB + 1mL E coli + 1mL 5.3 phage stock
2. Liquid culture purification - 1(7.15)
1) For each infected test tubes (10uL, 100uL, 1mL), put 1mL of liquid culture into 5 eppendorf tubes.
2) Centrifuge at 3000 rpm for 5 minutes
3) Transfer supernatant into new eppendorf tubes. 5 eppendorf tubes for each phage concentration.
4) Add 100 uL of chloroform to each of the new tubes and gently shake
5) We labeled the purified stock as 7.15
3. Titer to determine phage concentration - 1(7.15)
1) For each concentration of phage, specifically 10uL, 100uL, and 1mL, 1:100 dilution series were performed to generate 0, -2, -4, -6. 1:10 dilution series were then performed to generate -7, -8, and -9.
2) For each dilution, a test tube was assigned to it. To each test tube, 0.75mL of BL21 liquid culture overnight was added and then transfected with 30uL of phage dilution. After 20 minutes of incubation, 7mL of x8 agar was added to each test tube and the content was then plated.
3) Plates were incubated upside down for 24 hours.
4. Set up phage liquid culture - second round of propagation (7.17)
- phage: 4mL LB + 1mL E coli
5uL phage: 4mL LB + 1mL E coli + 5μL 5.3 phage stock
10uL phage: 4mL LB + 1mL E coli + 10μL 5.3 phage stock
5. Liquid culture purification (7.19)
1) For each infected test tubes (5uL, 10uL, 1mL), put 1mL of liquid culture into 5 eppendorf tubes.
2) Centrifuge at 3000 rpm for 5 minutes
3) Transfer supernatant into new eppendorf tubes. 5 eppendorf tubes for each phage concentration.
4) Add 100 uL of chloroform to each of the new tubes and gently shake
5) We labeled the purified stock as 7.19
6. Titer to determine phage concentration (7.19)
1) For each concentration of phage, specifically 5uL and 10uL, 1:100 dilution series were performed to generate 0, -2, -4, -6. 1:10 dilution series were then performed to generate -7, -8, and -9.
2) For each dilution, a test tube was assigned to it. To each test tube, 0.75mL of BL21 liquid culture overnight was added and then transfected with 30uL of phage dilution. After 20 minutes of incubation, 7mL of x8 agar was added to each test tube and the content was then plated.
3) Plates were incubated upside down for 24 hours.

V) Results

1. Set up phage liquid culture - first round of propagation
2. Titer to determine phage concentration - 1
3. Set up phage liquid culture - first round of propagation
4. Titer to determine phage concentration - 1

VI) Conclusion/Next Step